Derivatives of L-amino acyl L-carnitine, process for their preparation pharmaceutical compositions having hepatoprotecting activity containing same

ABSTRACT

L-aminoacyl derivatives of L-carnitine of general formula (I) ##STR1## wherein R is an alkyl radical selected from 1-methyl-propyl, isobutyl, isopropyl, mercaptomethyl and 3-guanidino propyl, and their pharmacologically acceptable salts, are prepared e.g. by reacting a solution in an organic solvent of L-carnitine whose carboxyl group is protected with an N-protected aminoacid in the presence of a condensing agent and then removing the amino-acid and carnitine protecting groups, thus obtaining the desired compound.

This is a divisional of co-pending application Ser. No. 07/067,694, filed on June 29, 1987, now U.S. Pat. No. 4,812,478.

The present invention relates to a novel class of L-amino acyl L-carnitines, the process for their preparation and the pharmaceutical compositions having hepatoprotecting activity comprising these compounds as active principles.

More particularly, the present invention relates to L-amino acyl-carnitines of general formula (I) ##STR2## wherein R is an alkyl radical selected from 1-methyl-propyl, isobutyl, isopropyl, mercaptomethyl and 3-guanidino propyl, and their pharmacologically acceptable salts.

Therefore, if the meanings of R are taken into account, the compounds specifically encompassed by the general formula (I) are: ##STR3##

It is apparent that the pharmacologically acceptable salts of the compounds of formula (I) may have the general formula (I') ##STR4## wherein X⁻ is the anion of a pharmacologically acceptable acid, such as for instance hydrochloric, bromidric, phosphoric, sulphuric and orotic acid; or they may have the general formula (I") ##STR5## wherein X⁻ has the above-identified meaning.

Since the salts (I") are more stable than both the salts (I') and the inner salts (I) and since in every case the conversion from the (I") or (I') salts into inner salts is carried out via known procedures (using e.g. ionic exchange resins whose selection will be obvious to any average skilled expert) for simplicity sake reference will be made hereinbelow to the salts of formula (I").

Acyl derivatives of L-carnitine are prepared by dissolving L-carnitine in trifluoroacetic acid and treating the resulting solution with the acid chloride of the desired acid. This synthesis route cannot be used for preparing the L-aminoacyl derivatives of L-carnitine of the present invention because:

(1) the activation of an aminoacid as acid chloride is only feasible upon previous protection of the NH₂ group with suitable protecting groups (e.g. acetyl and tosyl) whose subsequent removal requires such reaction conditions as to break the ester bond and/or lead to formation of unsatured by-products, such as crotonoylbetaine;

(2) the use of trifluoro acetic acid (the carnitine solvent of choice) brings about the instability and poor reactivity of the acid chloride of the protected aminoacid.

According to the present invention, the above-identified problems are overcome:

(1') by using N,N'-carbonyldiimidazole as activator of the aminoacid carboxyl group;

(2') by using, in place of trifluoroacetic acid, an inert organic solvent wherein, however, carnitine would be unsoluble.

In accordance with the present invention, this latter problem is solved by following either one of these alternatives routes:

(a) either synthesizing an ester of a carnitine salt which is soluble in the desired organic solvent and easily hydrolyzable after condensation with the amino acid for restoring the free carboxyl group; or

(b) using an L-carnitine precursor soluble in the desired organic solvent and subsequently converting the aminoacyl derivative of the precursor into L-carnitine aminoacyl derivative.

In accordance with the present invention, the L-amino acyl derivatives of L-carnitine of formula (I) are, therefore, prepared via two distinct synthesis routes depending on whether as starting material either the ester of an L-carnitine salt is used, preferably benzyl L-carnitine perchlorate (process A) or L- or D,L-norcarnitine tert-butyl ester (process B).

Specifically, process A comprises the following steps:

(a) reacting at 0° C.-30° C., for 0.5-24 hours, a benzyl L-carnitine salified with an anion y⁻ selected from perchlorate, tetraphenylborate and iodide in an inert anhydrous organic solvent selected from tetrahydrofurane and acetonitrile, with an L-aminoacid having its NH₂ group protected as N-carbobenzoxy, in the presence of N,N'-carbonyldiimidazole;

(b) substituting the anion X⁻ for the anion y⁻ by means of a weakly basic ion exchange resin by eluting the product in an alcoholic or aqueous-alcoholic solvent;

(c) removing the N-carbobenzoxy group of the aminoacid and the benzyl radical of benzyl L-carnitine by hydrogenation in the presence of a hydrogenation catalyst selected from 10% Pd/C and PtO₂ in an alcoholic, aqueous-alcoholic solvent or water at room temperature at a pressure of 1-4 kg/cm².

Preferably, the ion exchange resin of step (b) is AMBERLIST 21 activated in Cl⁻ form.

Process B comprises the following steps:

(a') reacting at 0° C.-30° C., for 4-24 hours L- or D,L-norcarnitine tert-butyl ester in a solvent selected from tetrahydrofurane and acetonitrile with an L-aminoacid having its NH₂ group protected as N-carbotertbutoxy in the presence of N,N'-carbonyl diimidazole;

(b') in the event D,L-norcarnitine tert-butylester has been used, separating the two diastereoisomers thus formed, L-N-carbotertbutoxy aminoacyl L-norcarnitine tertbutyl ester and L-N-carbotertbutoxy amino acyl D-norcarnitine tert butyl ester, via known procedures;

(c') methylating at 15° C.-30° C., for 4-24 hours the product obtained in step (a') or (b') with methyl iodide in an organic solvent selected from acetone and methyl ethyl ketone;

(d') removing the N-carbotertbutoxy group of the aminoacid and the tert-butyl radical in an acid environment, using trifluoroactic acid or a gaseous HCl solution in n inert solvent selected from chloroform and methylene chloride; and

(e') substituting the X⁻ anion for the I⁻ anion eluting an aqueous or alcoholic solution of the product of step (d') on a weakly basic ion exchange resin.

Preferably, the separation of step (b') is carried out either by chromatography on a silica column or by preparative HPLC.

Processes A and B are illustrated in the following reaction scheme. ##STR6##

The following non-limiting examples illustrate the preparation of some of the compounds of the present invention.

EXAMPLE 1 Preparation of L-leucyl L-carnitine chloride hydrochloride (ST 599) (Process A). (a) Preparation of N-carbobenzoxy L-leucyl L-carnitine benzyl ester perchlorate.

N-carbobenzoxy L-leucine (2.65 g; 0.01 moles) was dissolved in 10 cc of anhydrous tetrahydrofurane (THF). N,N'-carbonyl diimidazole (1.82 g; 0.012moles) at 0° C. was added to the solution. The resulting solution was kept under stirring at room temperature for half an hour. Then, a solution of L-carnitine benzyl ester perchlorate (3.5 g; 0.01 moles) in 5 cc of anydrous THF was added. The mixture was kept at room temperature for24 hours. To the filtered reaction mixture 10 cc of 10% Na₂ CO₃ were added. The solid thus formed was filtered off and the filtrate was diluted with 10 cc H₂ O and twice extracted with ethyl acetate. The organic phase was washed with 10 cc H₂ O, dried over Na₂ SO₄ and brought to dryness.

The oily residue thus obtained was dissolved in chloroform and washed with H₂ O. The chloroform concentrate yielded a residue of 3.3 g (yield about 55%). The product was examined via HPLC.

    ______________________________________                                         Column        Bondapak C.sub.18                                                Eluant        NH.sub.4 H.sub.2 PO.sub.4 0.05M--CH.sub.3 CN 60-40               Pressure      57 atm (58.881 kg/cm.sup.2)                                      Flow rate     2 ml/min                                                         Detector      UV λ 205                                                  Chart speed   0.5 cm/min                                                       Rt            17.66 minutes                                                    ______________________________________                                    

(b) Preparation of N-cargogenzoxy L-leucyl L-carnitine benzyl ester chloride.

N-carbobenzoxy L-leucyl L-carnitine benzylester perchlorate (3 g; 0.005 moles) was dissolved in methanol and the resulting solution passed througha column of 30 ml of AMBERLIST A 21 resin activated in Cl⁻ form. The resin was eluted with methanol. The concentrated methanol solution yielded2.5 g of a hydroscopic white solid (yield 95%).

(c) Removal of the protecting groups of N-carbobenzoxy L-leucyl L-carnitinebenzylester chloride.

N-carbobenzoxy L-leucyl L-carnitine benzyl ester chloride (2.5 g; 0.0047 moles) was dissolved in 25 cc H₂ O and hydrogenated with 0.5 g of 10%Pd/C under pressure (40 psi; 2.8 kg/cm²) at room temperature for 4 hours. The solution was filtered and 0.5 g of 10% Pd/C added to it; the hydrogenation was continued for 24 hours. At the end of the hydrogenation the aqueous solution was filtered and lyophilized. 1.2 g of a hygroscopic white solid were obtained (yield 80%). The product thus obtained was purified by preparative HPLC.

    ______________________________________                                         Chromatograph     Water Delta prep. 3000                                       Column            Prepak C.sub.18                                              Detector          R.I. Iota                                                    Recorder          Houston "Omniscribe"                                         Eluant            H.sub.2 O 100%                                               Flow rate         20 ml/min                                                    Column pressure   750 psi (52.7 kg/cm.sup.2)                                   Eluant pressure   40 psi (2.8 kg/cm.sup.2)                                     ______________________________________                                    

1 g of the product was dissolved in 20 ml H₂ O. The solution was filtered on W42 filter and injected into the chromatograph. The collected fractions were acidified and lyophilized; 350 mg of the title product wereobtained (yield 35%). The lyophilized product, washed with ethyl ether and dried, had the following analytical characteristics:

[α]₂₅ ^(D) =-6.6 (C=1, H₂ O)

Melting point=190° C. dec. (it softens at 110° C.)

TLC=CHCl₃, MetOH, NH_(4O) H; 50, 30, 8

Rf=0.1, I₂ detector

K.F.=2.5%

Elementary analysis: for C₁₃ H₂₈ N₂ O₄ Cl₂ : C 43.49%; H 9.76%; N 7.95%; Cl 20.59%

NMR D₂ O: 5.9 (1H, m ##STR7##4.2 (1H, t, ##STR8##3.8 (2H, m, N⁺ --CH₂ --); 3.3 (9H, s, (CH₃)₃ N⁺); 3.0 52H, d, --CH₂ --COOH); 2.2-1.8 (3H, m, CH₂ --CH); 1.0 (6H, d, CH--(CH₃)₂)

EXAMPLE 2 Preparation of L-valyl L-carnitine chloride hydrochloride (ST 601) (ProcessA) (a) Preparation of N-cargogenzoxy L-valyl L-carnitine benzyl ester perchlorate

N-carbobenzoxy L-valine (34 g; 0.13 moles) was dissolved in 130 cc of anhydrous THF. N,N'-carbonyl diimidazole (25 g; 0.15 moles) was added to the solution. The solution was kept under stirring at 0° C. for 30 minutes. Then, a solution of L-carnitine benzyl ester perchlorate (45 g; 0.13 moles) in 65 cc THF was added and the resulting solution was kept under stirring at room temperature for 24 hours. 130 cc of 10% Na₂ CO₃ were then added to the solution. After the solid thus formed was filtered off, the filtrate diluted with 150 cc H₂ O was twice extracted with 150 cc of ethyl acetate. The organic phase dried over anhydrous Na₂ SO₄ was concentrated under vacuum. The oily residue was dissolved in CH₂ Cl₂ and washed with H₂ O. The dried organic phase was concentrated to dryness yielding 52 g of a hygroscopic solid (yield 68%).

TLC: CHCl₃ 50, CH₃ OH 30, NH₄ OH 8; Rf=0.9

HPLC

Column: μBondapak C₁₈

Eluant: NH₄ H₂ PO₄ 0.05M--CH₃ CN 60-40

Pressure: 46 atm (47.518 kg/cm²)

Flow rate: 1 ml/min

Detector: UV λ=205; att. 4

Chart speed: 0.5 cm/min

Rt: 23.99 min

(b) Preparation of N-carbobenzoxy L-valyl L-carnitine benzyl ester chloride.

N-carbobenzoxy L-valyl L-carnitine benzyl ester perchlorate (52 g) was dissolved in 200 cc methanol and the resulting solution eluted through a column of 600 ml of A 21 AMBERLIST resin activated in Cl⁻ form. The eluate was concentrated under vacuum, thus obtaining 46 g of N-carbobenzoxy L-valyl L-carnitine benzyl ester chloride (yield 100%).

(c) Conversion of N-carbobenzoxy L-valyl L-carnitine benzyl ester chloride into L-valyl L-carnitine chloride hydrochloride.

N-carbobenzoxy L-valyl L-carnitine benzyl ester chloride (46 g; 0.088 moles) was dissolved in 100 cc H₂ O. 10 g of 10% Pd/C were added to the solution. The resulting reaction mixture was hydrogenated under pressure (24 psi; 1.68 kg/cm²) for 4 hours. Subsequently, further 10 g of catalyst were added to the reaction mixture and the hydrogenation wascontinued for 20 hours at 50 psi (3.51 kg/cm²); the solution was filtered and lyophilized. 23 g of the title compound were obtained (yield 88%). The compound was purified by preparative HPLC.

Chromatograph: Water delta prep. 3000

Column: Prepak C₁₈

Detector: R.I. Iota

Recorder: Houston "Omniscribe"

Eluant: H₂ O 100%

Flow rate: 20 ml/min

Column pressure: 750 psi (52.7 kg/cm²)

Eluant pressure: 40 psi (2.81 kg/cm²)

1 g sample was dissolved in 20 ml H₂ O, the solution filtered on W 42 filter and injected into the chromatograph.

The collected fractions were acidified with 1N HCl 400 mg of the title compound were obtained.

HPLC

Column: μBondapak NH₂

Pressure: 1000 psi (70.31 kg/cm²)

Flow rate: 1 ml/min

Eluant: KH₂ PO₄ 0.05N--CH₃ CN (35-65)

UV Detector: λ205; att. 30

Chart speed: 0.5 cm/min

Rt: 23.7 minutes

NMR D₂ O δ 5.8 (1H, m, ##STR9##4.3 (1H, d, --CH--NH₂); 4.0 (2H, m, N⁺⁻⁻ CH₂); 3.4 (9H, s, (CH₃)₃ N⁺); 2.9 (2H, d, CH₂ --COOH); 2.4-2.2 (1H, m, CO--CH--); 1.2 (6H, d, CH(CH₃)₂

[α]₂₅ ^(D) =-7.45 (c=1 H₂ O)

Melting point=160° C. dec (it softens at 110° C.)

TLC=CHCl₃, MetOH, NH₄ OH; 50, 30, 8

R_(F) =0.3; rivelatore I₂

K.F.=6.5%

Elementary analysis: for C₁₂ H₂₆ N₂ O₄ Cl₂ : C 40.78%; H 8.15%; N 8.03%; Cl 18.91.

EXAMPLE 3 Preparation of L-isoleucyl L-carnitine chloride (ST 583) (Process B) (a') Preparation of N-carbotertbutoxy L-isoleucyl D,L-norcarnitine tert-butylester.

N,N'-carbonyl diimidazole (2.7 g; 0.017 moles) was added at 0° C. toa solution of N-carbotertbutoxy L-isoleucine (2.4 g; 0.01 moles) in 10 cc anhydrous THF. To this solution kept under stirring at room temperature for 30 minutes under a nitrogen atmosphere, D,L-norcarnitine tert-butyl ester (2.03 g; 0.01 moles) dissolved in 5 cc THF was then added. This mixture was kept at room temperature for 24 hours. 10 cc of 10% Na₂ CO₃ were then added.

The resulting mixture was kept under stirring for 30 minutes and then filtered. The aqueous solution diluted with 10 cc H₂ O was twice extracted with 10 cc ethyl acetate. The organic phase, washed with H₂O, was concentrated under vacuum. An oil was obtained which washed with cyclohexane gave 2.3 g of a product. This product, examined by TLC (AcOEt 98-triethylamine 2, development ninidrine), showed two spots at Rf 0.77 and 0.84 corresponding to the two diasterisomers thus formed. The raw reaction product was subjected to preparative HPLC. The compound at lower Rf was isolated, corresponding to N-carbotertbutoxy L-isoleucyl L-norcarnitine tert-butyl ester (yield about 60%).

Chromatograph: Jobin Yvon; prep. 100 with SS column of 4 cm of diameter

Detector: KNAVER X 16 refractometer

Recorder: Houston Omniscribe

Resin: Lichropre SI 60 15-25 g 200

Eluant: ethyl acetate: 45%; chloroform: 55%

Column pressure: 12 atm (12.396 kg/cm²)

Eluant pressure: 6 atm (6.198 kg/cm²)

Flow rate: 30 ml/min

NMR CHCl₃ δ 5.4 (1H, m, ##STR10##5.0 (1H, d, --NH--); 4.2 (1H, m, --CH--NH--); 3.8 (2H, d, N⁺ --CH₂); 2.5-2.2 (2H, m, --CH₂ --COO+6H, s, (CH₃)₂ N); 1.8-1.2 (3H, m, CH--CH₂ CH₃ +18H, s, 2(CH₃)₃); 1.9 (6H, d, ##STR11##

(b') Preparation of N-carboterbutoxy L-isoleucy L-carnitine tert-butyl ester iodide;

15 cc methyl iodide were added to a solution of N-carbotertbutoxy L-isoleucyl L-norcarnitine tert-butyl ester (22 g; 0.053 moles) in 220 cc acetone. The solution was kept at room temperature for 4 hours and then concentrated to dryness under vacuum. 29 g of product (0.052 moles; yield 100%) were obtained.

TLC: CHCl₃ 50 MetOH 30 NH₄ OH 8 Rf 0.8

NMR: CDCl₃ δ 5.6 (1H, m, ##STR12##4.9 (1H, d, --NH--); 4.3-3.8 (3H, m, ##STR13## --CH₂ N⁺); 3.5 (9H, s, (CH₃)₃ N⁺); 2.0 (2H, d, CH₂ --COOH); 1.8-1.3 (18H, s, --COOC(CH₃)₃ ; NHCOOC(CH₃)₃ +3H, m, CH--CH--CH₂ --; CH₂ CH₃); 1.0 (6H, m, ##STR14##

(c') and (d') Conversion of N-carbotertbutoxy L-isoleucyl L-carnitine tert-butyl ester iodide into L-isoleucyl L-carnitine chloride.

N-carbotertbutoxy L-isoleucyl L-carnitine tert-butyl ester iodide (29 g; 0.052 moles) was dissolved in 96 cc trifluoroacetic acid and the solution kept under stirring at 0° C. for 2 hours. Ethyl ether was added to the solution until a yellow oil precipitated. The resulting suspension wasdecanted, the precipitate dissolved in H₂ O and the aqueous solution was extracted with ethyl ether three times. The aqueous solution was decolorized with active charcoal, filtered and eluted through a column of IR 45 AMBERLITE resin activated in Cl⁻ form. The eluate was lyophilized and 12 g (yield 66%) of product were obtained.

TLC: CHCl₃ 50, MetOH 30, NH₄ OH 8, Rf=0.3

The product was further purified via preparative HPLC.

Chromatograph: Jobin Yvon prep. 100 with SS column of 4 cm of diameter.

Detector: R.I. Knaver X 16

Recorder: HOUSTON "OMNISCRIBE" 0.5 cm/min

Resin: Lichroprep RP₁₈ 25-40 m 200 g

Eluant: H₂ O 100%

Column pressure: 10 atm (10.33 kg/cm²)

Eluant pressure: 3 atm (3.099 kg/cm²)

Flow rate: 28 ml/min

6 g of pure product were obtained.

NMR D₂ O δ 5.7 (1H, m, ##STR15##4.2-3.8 (3H, m, ##STR16##CH₂ --N⁺); 3.2 (9H, s, (CH₃)₃ N⁺); 2.7 (2H, d, CH₂ --COOH); 2.1 (1H, m, ##STR17##1.3 (2H, t, CH₂ CH₃); 0.9 (6H, m, ##STR18##HPLC: Varian Column: μBondapack NH₂

Eluant: KH₂ PO₄ 0.05N--CH₃ CN (35-65); flow rate 1 ml/min

Detector: UV LC 75; λ205; att. 4

Integrator: 4270 Varian

Chart speed: 0.5 cm/min

Rt: 18.65 minutes

[α]₂₅ ^(D) =+1.8 (c=1, H₂ O)

Melting point=129° C. dec.

K.F.=6.8%

Elementary analysis: for C₁₃ H₂₇ N₂ O₄ Cl: C 47.90%; H 8.98%; N 8.84%; Cl 11.49%.

EXAMPLE 4 Preparation of L-arginyl L-carnitine chloride hydrochloride. (Process A) (a) Preparation of N.sub.α, N.sub.δ, N.sub.ω -tricarbobenzoxy L-arginyl L-carnitine benzyl ester perchlorate.

N.sub.α, N.sub.δ, N.sub.ω -tricarbobenzoxy L-arginine (57.6 g; 0.1 moles) was dissolved in 100 cc anhydrous THF. To the solution, N,N'-carbonyl diimidazole (15 g; 0.11 moles) was added. The solution was kept under stirring at room temperature for 45 minutes. Then,dimethyl amino-pyridind (1.2 g; 0.01 moles) and a solution of L-carnitine benzyl ester perchlorate (35 g; 0.1 moles) in 50 cc THF were added. The resulting solution was kept under stirring at room temperature for 48 hours and then concentrated under vacuum. The residue was dissolved in CH₂ Cl₂ and washed with 1% HCl. The organic phase was dried overanhydrous Na₂ SO₄ and concentrated under vacuum. 73 g of a hygroscopic solid (yield 80%) were obtained.

HPLC

Column: Lichrosorb RP-8

Eluant: KH₂ PO₄ 0.05M--CH₃ CN 40-60

Pressure: 57 atm (58.881 kg/cm²)

Flow rate: 1 ml/min

Detector: UV λ205

Chart speed: 0.5 cm/min

Rt: 11.07 minutes

(b) Preparation of N.sub.α, N.sub.δ, N.sub.ω -tricarbobenzoxy L-arginy L-carnitine benzyl ester chloride.

N.sub.α, N.sub.δ, N.sub.ω -tricarbobenzoxy L-arginyl L-carnitine benzylester perchlorate (75 g; 0.08 moles) was dissolved in methanol and the resulting solution fed at the top of a column containing 750 ml of A 21 AMBERLIST resin activated in Cl⁻ form. The resin was eluted with methanol. The concentrated methanol solution yielded 68 g of ahygroscopic white solid (yield 95%). The product thus obtained was purifiedvia preparative HPLC.

Chromatograph: waters Delta prep 3000

Column: Prepak C₁₈ a 750 psi

Eluant: CH₃ CN 70: H₂ O 30

Flow rate: 30 ml/min

2 g of product were dissolved in 20 ml CH₃ CN, filtered through a W 42filter and injected into the chromatograph. The collected fractions were concentrated under vacuum and subjected to HPLC examination at the same conditions outlined at point (a).

The fractions with R_(t) =10.86 were combined and 32 g (yield 47%) of pure product were obtained.

(c) Removal of protecting groups from N.sub.α, N.sub.δ, N.sub.ω -tricarbobenzoxy L-arginyl L-carnitine benzyl ester chloride.

N.sub.α, N.sub.δ, N.sub.ω -tricarbobenzoxy L-arginyl L-carnitine benzyl ester chloride (4.2 g; 0.005 moles) was dissolved in 50cc H₂ O. 1.5 cc concentrated HCl were added to the solution. The resulting solution was hydrogenated with 1 g of 10% Pd/C under pressure (40 psi; 2.8 kg/cm²) at room temperature for 24 hours. The reaction mixture was filtered and 1 g of 1% Pd/C were added to the filtrate; the hydrogenation was continued for 24 hours.

When the hydrogenation ended, the reaction mixture was filtered and the filtrate was lyophilized. 2 g of a hygroscopic white solid were obtained (yield 86%). The product thus obtained was purified via preparative HPLC.

Chromatograph: Waters delta prep. 3000

Column: Prepak C₁₈

Detector: R.I. Iota

Recorder: Houston "Omniscribe"

Eluant: H₂ O 100%

Flow rate: 20 ml/min

Column pressure: 750 psi (52.7 kg/cm²)

Eluant pressure: 40 psi (2.8 kg/cm²)

1 g of the product was dissolved in 20 ml H₂ O, the solution filtered through W 42 filter and injected into the chromatograph. The collected fractions were acidified and lyophilized; 500 mg of the title product wereobtained (yield 35%). The lyophilized product, washed with ethyl ether and dried, showed the following analytical characteristics:

[α]₂₅ ^(D) =-6.6 (C=1, H₂ O)

TLC=CHCl₃, MetOH, NH₄ OH; 50, 30, 8

R_(F) =0.1, I₂ detector

NMR=D₂ O δ 5.7 (1H, m, ##STR19##4.3 (1H, m, ##STR20##3.8 (2H, m, N⁺ CH₂ --) 3.3 (11H, S, 5CH₃)₃ N⁺ --,CH₂ --NH); 2.8 (2H, d, --CH₂ COOH); 1.8 (4H, m, --CH₂ --CH₂ --)

The hepatoprotecting activity of the compounds was evaluated toward ethionine- and ammonium acetate-induced intoxication. It was found that the compounds are active both orally and parenterally at a dose equal to or lower than 10 mg/kg. Moreover, in vitro tests have shown that they are able to keep the structural and functional integrity of liver cells and mitochondria towards hexogenous noxae at nanomolar and micromolar concentrations.

Following single or repeated administrations for 15 days the compounds did not induce any toxic or lethal effect up to a dose of 1 g/kg orally or parenterally.

These compounds are, therefore, active for the therapeutical treatment of hepatic diseases which severely impair liver function.

The orally of parenterally administrable compositions which contain one of compounds of the present invention as active principle (e.g. tablets, capsule and injectable vials) are compounded with the usual excipients viaprocedures well known to the average skilled expert in pharmaceutical technology. 

What is claimed is:
 1. A method for providing hepatoprotection comprising administering, to a patient with a heparic disorder which impairs liver function, an effective amount of a composition comprising a compound of the formula I ##STR21## wherein R is an alkyl radical selected from the group consisting of 1-methyl-propyl, isobutyl, isopropyl, mercaptomethyl and 3-guanidinopropyl, and their pharmacologically acceptable salts, and a pharmaceutically acceptable carrier.
 2. The method, as in claim 1, wherein the composition is administered orally or parenterally.
 3. The method, as in claim 2, wherein the effective amount comprises a dose of 10 mg/kg or less of the compound.
 4. The method, as in claim 2, wherein the composition is administered in a single dose, or a repeated dose for up to 15 days.
 5. A method for providing hepatoprotection comprising administering, to a patient with a hepatic disorder which impairs liver function, an effective amount of a composition comprising a compound of the formula I' ##STR22## wherein R is an alkyl radical selected from the group consisting of 1-methyl-propyl, isobutyl, isopropyl, mercaptomethyl and 3-guanidinopropyl, and their pharmacologically acceptable salts, and X⁻ is the anion of a pharmacologically acceptable acid selected from the group consisting of hydrochloric, bromidic, phosphoric, sulphuric and orotic acid, and a pharmaceutically acceptable carrier.
 6. A method for providing heptoprotection comprising administering, to a patient with a hepatic disorder which impairs liver function, an effective amount of a compound of the formula I" ##STR23## wherein R is an alkyl radical selected from the group consisting of 1 methyl-propyl, isobutyl, isopropyl, mercaptomethyl and 3-guanidinopropyl, and their pharmacologically acceptable salts, and X⁻ is the anion of a pharmacologically acceptable acid selected from the group consisting of hydrochloric, bromidic, phosphoric, sulphuric and orotic acid and a pharmaceutically acceptable carrier. 